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体外区分真正的雄激素受体抑制与细胞毒性介导的报告基因转录激活减少。

Differentiating true androgen receptor inhibition from cytotoxicity-mediated reduction of reporter-gene transactivation in-vitro.

机构信息

Chemical Food Safety, Nestlé Research Centre, P.O. Box 44, CH-1000 Lausanne 26, Switzerland.

Chemical Food Safety, Nestlé Research Centre, P.O. Box 44, CH-1000 Lausanne 26, Switzerland.

出版信息

Toxicol In Vitro. 2017 Dec;45(Pt 3):359-365. doi: 10.1016/j.tiv.2017.03.014. Epub 2017 Apr 1.

DOI:10.1016/j.tiv.2017.03.014
PMID:28377212
Abstract

In vitro effect-based reporter assays are applied as biodetection tools designed to address nuclear receptor mediated-modulation. While such assays detect receptor modulating potential, cell viability needs to be addressed, preferably in the same well. Some assays circumvent this by co-transfecting a second constitutively-expressed marker gene or by multiplexing a cytotoxicity assay. Some assays, such as the CALUX®, lack this feature. The cytotoxic effects of unknown substances can confound in vitro assays, making the interpretation of results difficult and uncertain, particularly when assessing antagonistic activity. It's necessary to determine whether the cause of the reporter signal decrease is an antagonistic effect or a non-specific cytotoxic effect. To remedy this, we assessed the suitability of multiplexing a cell viability assay within the CALUX® transcriptional activation test for anti-androgenicity. Tests of both well-characterized anti-androgens and cytotoxic compounds demonstrated the suitability of this approach for discerning between the molecular mechanisms of action without altering the nuclear receptor assay; though some compounds were both cytotoxic and anti-androgenic. The optimized multiplexed assay was then applied to an uncharacterized set of polycyclic aromatic compounds. These results better characterized the mode of action and the classification of effects. Overall, the multiplexed protocol added value to CALUX test performance.

摘要

基于体外效应的报告基因检测方法可作为生物检测工具,用于检测核受体介导的调节作用。虽然这些检测方法可以检测到受体的调节潜力,但需要解决细胞活力问题,最好在同一孔中进行。一些检测方法通过共转染第二个组成型表达的标记基因或多重细胞毒性检测来规避这个问题。然而,一些检测方法,如 CALUX,缺乏这种功能。未知物质的细胞毒性会干扰体外检测,使结果的解释变得困难和不确定,特别是在评估拮抗活性时。有必要确定报告基因信号下降的原因是拮抗作用还是非特异性细胞毒性作用。为了解决这个问题,我们评估了在 CALUX 转录激活检测中,将细胞活力检测与抗雄激素活性进行多重检测的适用性。对两种经过充分研究的抗雄激素和细胞毒性化合物的测试证明,这种方法适用于在不改变核受体检测的情况下区分作用机制;尽管一些化合物同时具有细胞毒性和抗雄激素作用。然后,我们将优化的多重检测方法应用于一组未表征的多环芳烃化合物。这些结果更好地描述了作用模式和效应分类。总的来说,多重检测方案为 CALUX 检测性能增加了价值。

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